Quantitative Determination of Metabolic Fluxes during Coutilization of Two Carbon Sources: Comparative Analyses with Corynebacterium glutamicum during Growth on Acetate and/or Glucose

doi:10.1128/JB.182.11.3088-3096.2000

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Journal of Bacteriology, June 2000, p. 3088-3096, Vol. 182, No. 11
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Quantitative Determination of Metabolic Fluxes during Coutilization of Two Carbon Sources: Comparative Analyses with Corynebacterium glutamicum during Growth on Acetate and/or Glucose

Volker F. Wendisch,^* Albert A. de Graaf, Hermann Sahm, and Bernhard J. Eikmanns

Institute of Biotechnology 1, Research Center Jülich, D-52425 Jülich, Germany

Received 18 October 1999/Accepted 6 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Growth of Corynebacterium glutamicum on mixtures of the carbon sources glucose and acetate is shown to be distinct from growthon either substrate alone. The organism showed nondiauxic growthon media containing acetate-glucose mixtures and simultaneouslymetabolized these substrates. Compared to those for growth onacetate or glucose alone, the consumption rates of the individualsubstrates were reduced during acetate-glucose cometabolism, resultingin similar total carbon consumption rates for the three conditions.By ¹³C-labeling experiments with subsequent nuclear magnetic resonanceanalyses in combination with metabolite balancing, the in vivoactivities for pathways or single enzymes in the central metabolismof C. glutamicum were quantified for growth on acetate, on glucose,and on both carbon sources. The activity of the citric acid cyclewas high on acetate, intermediate on acetate plus glucose, andlow on glucose, corresponding to in vivo activities of citratesynthase of 413, 219, and 111 nmol · (mg of protein)¹ · min¹, respectively. The citric acid cycle was replenished by carboxylationof phosphoenolpyruvate (PEP) and/or pyruvate (30 nmol · [mg ofprotein]¹ · min¹) during growth on glucose. Although levels of PEP carboxylaseand pyruvate carboxylase during growth on acetate were similarto those for growth on glucose, anaplerosis occurred solely bythe glyoxylate cycle (99 nmol · [mg of protein]¹ · min¹). Surprisingly, the anaplerotic function was fulfilled completelyby the glyoxylate cycle (50 nmol · [mg of protein]¹ · min¹) on glucose plus acetate also. Consistent with the predictionsdeduced from the metabolic flux analyses, a glyoxylate cycle-deficientmutant of C. glutamicum, constructed by targeted deletion of theisocitrate lyase and malate synthase genes, exhibited impairedgrowth on acetate-glucosemixtures.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

In their natural environments microorganisms often encounter situations when not a single carbon source but mixtures of carbonand energy sources are present. Under such conditions, bacteriaoften utilize one carbon source preferentially, with the furthercarbon source(s) being consumed only, when the preferred one isexhausted. As already shown by Monod (29), the preferred carbonsource in general supports the best growth rate and/or growthyield, and the successive utilization of the substrates is oftenrepresented by a biphasic growth behavior (29). The classicalexample of this phenomenon is the diauxic growth of Escherichiacoli on glucose plus lactose, and the study of the underlyingprinciples initiated the era of research on gene regulation. Onthe other hand, by analysis of growth and carbon source consumption,it was shown that, e.g., Leuconostoc oenos cometabolizes glucosewith citrate or fructose (38). Also, E. coli cometabolizes hexosesunder carbon limitation conditions (reviewed in reference 20).Several other bacteria use two carbon sources in parallel (reviewedin reference 16); among these is Corynebacterium glutamicum,a gram-positive bacterium known for its ability to excrete aminoacids. C. glutamicum grows aerobically on a variety of carbohydratesand organic acids as carbon sources (23). The organism cometabolizesglucose and fructose, glucose and lactate, and glucose and pyruvate(6, 7), whereas it shows diauxic growth on glucose-glutamatemixtures (21). The carbon sources glucose and acetate have beenshown to serve as substrates for amino acid production by C. glutamicum(17). There is considerable knowledge about the enzymes andgenes involved in acetate and glucose metabolism as well as theirregulation (35, 36, 52, 53), whereas neither growth onacetate-glucose mixtures nor metabolite fluxes during growth onacetate have been studied indetail.

The utilization of acetate involves its uptake and subsequent activation to acetyl coenzyme A (acetyl-CoA) and, when acetateis the sole carbon source, also requires the operation of theglyoxylate cycle as an anaplerotic pathway (5). The key glyoxylatecycle enzymes isocitrate lyase and malate synthase have been purifiedfrom C. glutamicum, and biochemical characterization showed thatboth enzymes are subject to allosteric regulation by several intermediatesof the central metabolism (35, 36). In addition, the genesencoding isocitrate lyase (aceA) and malate synthase (aceB), aswell as the operon coding for the acetate-activating enzymes acetatekinase and phosphotransacetylase (the pta-ack operon), have beenisolated and characterized, and, by gene-directed mutagenesisand analysis of the mutants, all four enzymes have been shownto be essential for the growth of C. glutamicum on acetate asthe sole carbon and energy source (35, 36, 37). Furtherstudies revealed that all four enzymes are coordinatedly and specificallyup-regulated by the presence of acetate in the growth medium,and in all four cases, cat fusion and Northern blot experimentsrevealed that this regulation is due to transcriptional controlof the respective genes (37, 53).

The tight regulation of the enzymes involved in acetate metabolism of C. glutamicum is expected to cause significant changesof the carbon flux within the central metabolism of this organismwhen acetate instead of glucose is the sole carbon source. Althoughthe up-regulation of the enzymes during growth on acetate or onacetate-glucose mixtures (53) suggests that the respective pathwayscould also be active under this condition, this cannot be regardedas proof for in vivo activities and certainly cannot be used topredict the in vivo fluxes quantitatively. Not only have ¹³C-labeling experiments been used to identify metabolic pathways(see, e.g., references 24, 25, and 43), but by quantitativeanalyses of positional isotopic labeling information Walsh andKoshland (50) pioneered the determination of relative metabolicfluxes (reviewed in reference 19). The combination of metabolitebalancing and ¹³C-labeling experiments allowed the quantification of absolutemetabolite fluxes within the cellular central metabolism (see,e.g., references 26 and 41). In order to study the cometabolismof acetate plus glucose by C. glutamicum in a quantitative manner,we performed ¹³C-labeling experiments in combination with nuclear magnetic resonance(NMR) analyses and metabolite balancing to determine the in vivoactivities of pathways or single enzymes in the central metabolism,with a particular focus on the tricarboxylic acid (TCA) cycleand anaplerosis. From the flux analysis results, a hypothesisregarding the physiological significance of the glyoxylate cyclefor C. glutamicum was deduced and testedexperimentally.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Materials. Sodium [1-¹³C]acetate (99% atom enrichment) was purchased from Cambridge Isotope Laboratories, Andover, Mass., D-[5-¹³C]glucose (99% atom enrichment) from Isotec, Miamisburg, Ohio,and sodium 3-trimethylsilyl-[2,2',3,3'-D₄]propionate (99% atomenrichment) from Aldrich Chemicals, Milwaukee,Wis.

Microorganisms and cultivation conditions. The wild-type (WT) strain of C. glutamicum ATCC 13032 and the isocitrate lyase- and malate synthase-negative double mutantC. glutamicum WT $Delta$ AB, described in this work, were used. All C.glutamicum strains were precultured on Luria-Bertani complex medium(39), with kanamycin (50 µg/ml) added when appropriate. Exponentiallygrowing cells were harvested by centrifugation (5,000 × g, 5 min,4°C), washed twice in 50 mM NaCl-50 mM Tris-HCl (pH 6.3), andused to inoculate CgC minimal medium (11). The carbon and energysources were either unlabeled sodium acetate and/or glucose atthe concentrations indicated in Results or, for the ¹³C-labeling experiments, sodium [1-¹³C]acetate (99% atom enrichment) (10 g/liter), [5-¹³C]glucose (99% atom enrichment) (20 g/liter), or sodium [1-¹³C]acetate (99% atom enrichment) plus unlabeled glucose (10 g/litereach). All cultivations were done as 60-ml cultures in 500-mlbaffled Erlenmeyer flasks at 30°C and with agitation at 140 rpm.After about 4 generations, exponentially growing cells were harvestedand washed as described above. The cell pellet was then used forthe extraction of aminoacids.

Extraction, purification, and quantification of amino acids. Amino acids were extracted by acid hydrolysis of cell pellets and purified by cation-exchange chromatography as describedpreviously (31). They were quantified by reversed-phase liquidchromatography with precolumn ortho-phthaldialdehyde derivatization(42).

NMR spectroscopy. High-resolution ¹H NMR spectra of amino acids were obtained on an AMX-400 WB spectrometer (Bruker, Karlsruhe, Germany) operatingat 400.13 MHz and equipped with a multichannel interface and a5-mm inverse probehead. ¹³C enrichments were determined using the parameters and the methodsdescribed previously (44, 52).

Quantitation of metabolite fluxes. For the quantitation of carbon fluxes in the central metabolism of C. glutamicum, NMR spectroscopic and metabolite balancingdata were combined in a nonlinear least-squares fitting procedureas described previously (26, 27, 28, 45). C. glutamicumwas cultured on labeled carbon sources, and the ¹³C-labeling patterns of amino acids purified from exponentiallygrowing cells were determined. The ¹³C-labeling patterns of the precursors pyruvate, oxaloacetate,2-oxoglutarate, and 3-phosphoglycerate were deduced from the labelingpatterns of alanine and valine, threonine and aspartate, glutamateand arginine, and serine and glycine, respectively. For flux calculations,a representation of the central metabolism of C. glutamicum essentiallyaccording to that described by Marx et al. (26) was used. The(sets of) enzyme reactions and metabolite pools used to constructthe model are listed in Table 1. The precursor requirements forC. glutamicum biomass synthesis were taken from Marx et al. (26)except that, since in our experiments leucine was not supplemented,the precursor requirements were calculated based on the determinedleucine content of 439 µmol · (g [dry weight])¹. Flux calculations were based on the mathematical approach andthe computational tools described by Wiechert and de Graaf (54,55). The metabolic steady-state condition in the carbon fluxanalyses presented is based on the exponential growth of batchcultures. Precultivation was optimized such that the growth on¹³C-labeled carbon sources was exponential without an initial lagphase. To account for the unlabeled carbon content in the harvestedcells derived from the inoculum (i.e., 5%), the ¹³C label of the positionally labeled carbon source was corrected(i.e., 94.9% instead of 99.9% [5-¹³C]glucose) as has been described previously (26).

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TABLE 1. Description of fluxes and metabolites constituting the flux model of C. glutamicum

Construction of the isocitrate lyase- and malate synthase-deficient C. glutamicum WT $Delta$ AB. To generate a glyoxylate cycle-deficient mutant strain of C. glutamicum WT, the chromosomal region comprising the genes aceAand aceB, coding for isocitrate lyase and malate synthase, respectively,was deleted using standard methods (40). For the constructionof the gene replacement vector pK19mobsacB-3'AB3', the 3'-terminalparts of genes aceA and aceB were amplified using the PCR CoreKit from Boehringer Mannheim according to the manufacturer's instructions.To amplify the 3'-terminal region of aceB and aceA, primers VW1and VW2 and primers VW3 and VW4, respectively, were used. Thesequences of the primers are as follows (underlined nucleotidesare derived from the aceA-aceB locus, and boldfaced nucleotidescorrespond to either a BamHI, an EcoRI, or an XbaI restrictionsite): VW1, 5'-CGGGATCCGCCATGATGTTG-3' (nucleotides [nt]2567 to 2584 in EMBL accession no. 78491); VW2, 5'-CGGAATTCGCATCATCACCATTG-3'(nt 3021 to 3005 in EMBL accession no. 78491); VW3, 5'-CGGGATCCGCAGGCTACTTCGAC-3'(nt 1719 to 1734 in EMBL accession no. 75504); VW4, 5'-GCTCTAGAAGTTGGGTTCTGAGAAG-3'(nt 2170 to 2151 in EMBL accession no. 75504). The amplificationproducts were subcloned into vector pGEM-T (Promega), resultingin the vectors pGEM-T-aceA3' and pGEM-T-aceB3', respectively.In the next step, the 1.6-kb BamHI-ScaI fragment of pGEM-T-aceA3'was ligated with the 2.3-kb BamHI-ScaI fragment of pGEM-T-aceB3',resulting in vector pGEM-T-3'AB3'. Vector pGEM-T-3'AB3' containsthe 3'-terminal regions of genes aceA and aceB adjacent to eachother and in opposite directions. The 0.9-kb XbaI-EcoRI fragmentof pGEM-T-3'AB3' was ligated into the XbaI- and EcoRI-restrictedgene replacement vector pK19mobsacB (40), which is not replicablein C. glutamicum. Applying the procedure described by Peters-Wendischet al. (30), the resulting vector pK19mobsacB-3'AB3' was usedto delete the chromosomal aceA-aceB locus. The deletion of thechromosomal aceA-aceB locus was verified by Southern blot hybridization(data not shown). The aceA-aceB mutant was designated C. glutamicumWT $Delta$ AB. When it was grown on minimal medium containing either glucoseor glucose plus acetate, neither isocitrate lyase nor malate synthaseactivity could be detected in crude extracts (data not shown),thus proving that the respective genes in C. glutamicum WT $Delta$ ABhad in fact been knockedout.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Characterization of the growth of C. glutamicum on acetate, glucose, and acetate-glucose mixtures. C. glutamicum WT was cultured on CgC minimal medium containing various concentrations of acetate (20 to 180 mM) plus glucose(5 to 110 mM). The growth of C. glutamicum on all acetate-glucosemixtures was monophasic; an example is shown in Fig. 1. The concentrationsof both substrates in the culture broth decreased concomitantly,indicating that they were metabolized simultaneously. Thus, itwas likely that the parameters characterizing the growth of C.glutamicum on mixtures of glucose and acetate are distinct fromthose for cells growing on either carbon source alone. In comparativegrowth experiments with C. glutamicum WT on CgC minimal mediacontaining acetate and/or glucose, the growth rates, the biomassyields, and the substrate uptake rates were determined (Table2). On glucose as a sole carbon source, but not on acetate oron acetate-glucose mixtures, the dependence of the growth rateon the substrate concentration followed Monod kinetics, with amaximal growth rate of 0.38 h¹ and a half-maximal growth rate at 4.5 mM glucose. In the presenceof acetate in the medium, the growth rate decreased with increasingacetate concentrations (from about 0.32 h¹ at 60 mM acetate to about 0.24 h¹ at 180 mM acetate), probably reflecting the detrimental effectof acetate as an uncoupler of the transmembrane pH gradient (2).Comparison of the growth rates on acetate, acetate plus glucose,and glucose showed that the growth rate on acetate was lower thanthat of cells growing on glucose or glucose-acetate mixtures (Table2). The biomass yield (calculated as grams of carbon [C] [dryweight] per grams of C in the substrate) for growth of C. glutamicumon any acetate-glucose mixture was the same as that for growthon glucose alone, whereas that for growth on acetate was significantlylower (Table 2). During growth on acetate plus glucose, the acetateconsumption rate was always decreased compared to that for growthon acetate alone, as was the glucose consumption rate comparedto that for growth on glucose as the sole carbon source (Table2). Interestingly, the consumption rate of total carbon was similarunder the three conditions (about 900 to 1,100 nmol of C · [mgof protein]¹ · min¹). Thus, simultaneous utilization of acetate and glucose by C.glutamicum is clearly distinct from growth on either substratealone, and discernible carbon fluxes in the central metabolismshould reflect these differences.

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FIG. 1. Growth of C. glutamicum WT on mineral medium with 35 mM glucose and 120 mM acetate.

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TABLE 2. Growth characteristics of C. glutamicum grown on minimal medium with sodium [1-¹³C]acetate, sodium [1-¹³C]acetate plus unlabeled glucose, or [5-¹³C]glucose as the carbon and energy source

Quantitative determination of metabolite fluxes in C. glutamicum during growth on acetate, glucose, and a mixture of acetate and glucose. In order to quantify metabolic fluxes in the central metabolism of C. glutamicum, we performed ¹³C-labeling experiments combined with metabolite balancing as describedin Materials and Methods. C. glutamicum WT was cultured on minimalmedium with either sodium [1-¹³C]acetate, [5-¹³C]glucose, or a mixture of sodium [1-¹³C]acetate and unlabeled glucose as the sole carbon source. Thegrowth characteristics of the three cultures are summarized inTable 2. No significant by-product formation was detected inNMR analyses of culture supernatants. Exponentially growing cellsof the cultures were harvested and hydrolyzed, and amino acidswere purified from the lysate by liquid chromatography. The ¹³C-labeling patterns of alanine and valine, aspartic acid and threonine,glutamic acid and arginine, and serine and glycine were determinedby NMR, and the corresponding labeling patterns of pyruvate, oxaloacetate,2-oxoglutarate, and 3-phosphoglycerate were deduced (Table 3).Using these data, those for biomass accumulation, and those foracetate, glucose, and acetate-plus-glucose consumption, the invivo carbon metabolite fluxes within the central metabolism ofC. glutamicum were then quantitatively determined as summarizedin Fig. 2, 3, and 4, respectively.

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TABLE 3. ¹³C enrichments in carbon atoms of central metabolites of C. glutamicum WT cultured on CgC mineral medium containing [1-¹³C]acetate, [5-¹³C]glucose, or [1-¹³C]acetate plus unlabeled glucose

In C. glutamicum cells growing on acetate as a sole carbon source, the acetate was activated to acetyl-CoA with a specificactivity of 540 mU · (mg of protein)¹ (Fig. 2). About 5% of the acetyl-CoA was used directly in anabolicreactions, e.g., for fatty acid synthesis, whereas 18% was convertedby malate synthase in the glyoxylate cycle and 76% was convertedby citrate synthase and aconitase to isocitrate. Isocitrate wasmetabolized to about 24% via isocitrate lyase in the glyoxylatecycle, whereas the rest was further oxidized in the reactionsof the citric acid cycle. The malate formed by the glyoxylatecycle (99 mU · [mg of protein]¹) served to replenish the citric acid cycle. The majority (72mU · [mg of protein]¹, i.e., 73%) of biosynthetic precursors withdrawn from the citricacid cycle was used for the generation of cell material derivedfrom phosphoenolpyruvate and/or pyruvate (PEP/pyruvate)- and glyceraldehyde-3-phosphate.In summary, metabolization of acetate by C. glutamicum is characterizedby a high in vivo activity of the citric acid cycle, a high invivo activity of the glyoxylate cycle as the anaplerotic reaction,a high rate of PEP/pyruvate formation from oxaloacetate/malate,and gluconeogenesis with a 42-mU · (mg of protein)¹ conversion of PEP to glyceraldehyde-3-phosphate.

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FIG. 2. Metabolite fluxes in the central metabolism of C. glutamicum during growth on acetate. Fluxes are given in milliunits per milligram of protein. Fluxes for central metabolic pathways/reactions are boxed, fluxes towards biomass formation are given as pure numbers, and fluxes for exchange reactions are given in ovals. Abbreviations are as in Table 1.

In C. glutamicum cells growing on glucose as a sole carbon source, the glucose was consumed at a rate of 148 mU · (mg of protein)¹, about 25% of the glucose 6-phosphate was shuttled into biomassand CO₂ (directly, via fructose-6-phosphate, glyceraldehyde-3-phosphate,and pentose phosphate cycle intermediates), and the glycolyticflux from glyceraldehyde-3-phosphate to PEP/pyruvate was 227 mU· (mg of protein)¹ (Fig. 3). The formation of acetyl-CoA by pyruvate dehydrogenase(161 mU · [mg of protein]¹) amounted to about 70% of the PEP/pyruvate formation. Citratesynthase fueled acetyl-CoA into the citric acid cycle with anactivity of 111 mU · (mg of protein)¹, whereas about 30% of the acetyl-CoA was used as precursors,mainly for fatty acid synthesis. The glyoxylate cycle was inactiveduring the growth of C. glutamicum on glucose. The anapleroticreactions PEP carboxylase and pyruvate carboxylase replenishedthe citric acid cycle with a net conversion of PEP/pyruvate tooxaloacetate/malate of 30 mU · (mg of protein)¹. The combination of the [5-¹³C]glucose labeling experiment with metabolite balancing also allowedthe determination of exchange rates between glyceraldehyde-3-phosphateand PEP/pyruvate and between PEP/pyruvate and oxaloacetate/malate.The exchange rate in the interconversion of PEP/pyruvate and oxaloacetate/malatewas about twofold higher than the net flux of the carboxylatingreaction, i.e., the net conversion of PEP/pyruvate to oxalacetate-malate(30 mU · [mg of protein]¹) is the sum of the PEP/pyruvate carboxylation of 132 mU · (mgof protein)¹ and the simultaneously occurring malate-oxalacetate decarboxylationof 102 mU · (mg of protein)¹. Similarly, an interconversion of glyceraldehyde-3-phosphateand PEP/pyruvate of about four times the net conversion was found(i.e., the exchange rate was 469 mU · [mg of protein]¹ versus a net glyceraldehyde-3-phosphate formation of 227 mU ·[mg of protein]¹). To summarize, the central metabolism of C. glutamicum cellsgrowing on glucose is characterized by a low activity of the citricacid cycle, the absence of glyoxylate cycle activity, and anaplerosissolely by carboxylation of PEP or pyruvate.

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FIG. 3. Metabolite fluxes in the central metabolism of C. glutamicum during growth on glucose. Fluxes are given in milliunits per milligram of protein. Fluxes for central metabolic pathways/reactions are boxed, fluxes towards biomass formation are given as pure numbers, and fluxes for exchange reactions are given in ovals. Abbreviations are as in Table 1.

In C. glutamicum cells growing on a mixture of acetate and glucose, the consumption of both carbon sources (72 mU · [mg ofprotein]¹ for glucose and 270 mU · [mg of protein]¹ for acetate) was reduced approximately twofold compared to growthon either carbon source alone (Fig. 4). Acetyl-CoA was formedpredominantly by activation of acetate (270 mU · [mg of protein]¹) and only with 33 mU · (mg of protein)¹ by the pyruvate dehydrogenase complex. About 73% of the acetyl-CoAwas funneled into the citric acid cycle, and 11% was used directlyin biosynthetic reactions. Surprisingly, the glyoxylate cyclewas active under this growth condition, with isocitrate lyaseand malate synthase activities of 50 mU · (mg of protein)¹. Isocitrate was metabolized to 23% by isocitrate lyase, the restbeing oxidized by isocitrate dehydrogenase and the further reactionsof the citric acid cycle. The glyoxylate cycle provided malatenot only to replenish the citric acid cycle for intermediateswithdrawn for 2-oxoglutarate- and oxaloacetate-derived biosyntheses,but to an extent of 30% to generate PEP or pyruvate by decarboxylation.PEP carboxylase and pyruvate carboxylase did not serve an anapleroticfunction under this growth condition. During growth on glucoseplus acetate, the metabolization of glucose served primarily togenerate the precursors for biosyntheses derived from intermediatesof glycolysis and the pentose phosphate pathway. Taken together,the central metabolism of C. glutamicum cells growing on acetateplus glucose is characterized by a relatively low conversion rateof glucose to PEP/pyruvate, an intermediate activity of the citricacid cycle, and a glyoxylate cycle completely fulfilling the anapleroticfunction.

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FIG. 4. Metabolite fluxes in the central metabolism of C. glutamicum during growth on acetate plus glucose. Fluxes are given in milliunits per milligram of protein. Fluxes for central metabolic pathways/reactions are boxed, fluxes towards biomass formation are given as pure numbers, and fluxes for exchange reactions are given in ovals. Abbreviations are as in Table 1.

Construction and analysis of a glyoxylate cycle-deficient C. glutamicum strain. From the finding that in C. glutamicum cells growing on the mixture of acetate and glucose, the glyoxylate cycle completelyfulfills the anaplerotic function, it might be deduced that thiscycle is essential for the growth of C. glutamicum on minimalmedium containing both substrates. In order to test this hypothesis,we constructed and analyzed a defined glyoxylate-deficient C.glutamicum mutant. By gene-directed mutagenesis, the aceA andaceB genes, encoding isocitrate lyase and malate synthase, respectively,were deleted from the chromosome of C. glutamicum WT (see Materialsand Methods). The deletion of the chromosomal aceA-aceB locuswas verified by Southern blot hybridization (data not shown),and the aceA-aceB mutant was designated C. glutamicum WT $Delta$ AB. Incrude extracts of C. glutamicum WT $Delta$ AB grown in the presence ofacetate, neither isocitrate lyase nor malate synthase activitywas detectable (<0.01 U · [mg of protein]¹), whereas crude extracts of the parental strain, C. glutamicumWT, showed activities of both isocitrate lyase (1.05 U · [mg ofprotein]¹) and malate synthase (0.56 U · [mg of protein]¹). Comparative growth experiments on minimal media containingacetate, glucose, and acetate plus glucose as carbon sources wereperformed with C. glutamicum WT and the glyoxylate cycle-deficientstrain C. glutamicum WT $Delta$ AB. Both strains grew comparably wellon glucose, with growth rates of 0.33 and 0.31 h¹, respectively. In contrast to the parental WT strain, the glyoxylatecycle-deficient strain WT $Delta$ AB was not able to grow on acetate asa sole carbon source, corroborating our previous finding thatthe activities of isocitrate lyase and malate synthase are essentialfor growth on this substrate as a sole carbon source (36, 37).On minimal medium containing acetate plus glucose, C. glutamicumWT $Delta$ AB was able to grow; however, the growth rate was 0.27 h¹ compared to 0.34 h¹ (mean values from three independent cultivations by two determinationsper experiment with relative errors of less than 5%) for the parentalWT strain and thus was significantly lower. These results showthat the glyoxylate cycle is essential for optimal growth of C.glutamicum when both acetate and glucose are present in the growthmedium; however, they also show that the anaplerotic functionof the glyoxylate cycle can be partly taken over by PEP carboxylaseand/or pyruvatecarboxylase.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The carbon and energy source acetate can serve as a substrate in fermentative amino acid production with C. glutamicum (17).The quantitative determination of metabolic fluxes during thegrowth of C. glutamicum WT on acetate as a sole carbon sourcereported here complements flux analyses of different C. glutamicumstrains metabolizing either glucose or fructose (see, e.g., references8, 26, 27, 46). During growth on acetate, the acetateconsumption rate was in the range of 540 nmol · (mg of protein)¹ · min¹, which is much higher than expected from the previous kineticcharacterization of the acetate carrier in glucose-grown cells(9). However, in acetate-grown cells, it might well be thatthe acetate carrier gene is up-regulated, as are the acetate utilizationgenes in C. glutamicum (53). The low biomass yield on acetate(Table 2) indicated an increased energy metabolism, as most ofthe substrate carbon is oxidized to carbon dioxide. Consistently,the TCA cycle activity was high in vivo (isocitrate dehydrogenaseactivity in vivo, 314 mU · [mg of protein]¹ [Fig. 2]), which represents an increase of approximately threefoldcompared to growth on glucose (isocitrate dehydrogenase activityin vivo, 111 mU · [mg of protein]¹ [Fig. 3]). The increased generation of energy equivalents bythe TCA cycle satisfies the demand for gluconeogenesis and, moreover,might compensate for energy lost due to uncoupling of the membranepotential by acetate. Uncoupling by weak acids and its deleteriouseffect on growth have been demonstrated for E. coli and Clostridiumthermoaceticum (1, 2) and may explain our finding that growthrates of C. glutamicum on acetate decrease with increasing acetateconcentrations in themedium.

Acetate-glucose mixtures were coutilized by C. glutamicum and supported monophasic growth. During growth on glucose-acetatemixtures, the consumption rates for the individual carbon sourceswere reduced in such a way that the total carbon consumption wasabout the same as that during growth on either carbon source alone.This result indicates that either the uptake of acetate and ofglucose or the in vivo carbon fluxes from glucose to acetyl-CoAand from acetate to acetyl-CoA are directly or indirectly regulatedby the carbon source in the growth medium. In contrast to C. glutamicum,Azotobacter vinelandii preferentially uses acetate when grownon glucose-acetate mixtures, which is due to acetate-dependentinhibition of glucose uptake and glycolysis (15, 48). E. coli,too, does not coutilize glucose and acetate but preferentiallyuses glucose (4) due to carbon catabolite repression of theacetate-activating acetyl-CoA synthetase and probably also ofthe glyoxylate cycle enzymes isocitrate lyase and malate synthasein the presence of glucose (reviewed in reference 5). The metabolismof E. coli during growth on glucose-acetate mixtures is very similarin the first phase to growth on glucose as a sole carbon sourceand in the second phase to growth on acetate as a sole carbonsource (50, 51). To determine whether, for C. glutamicum,metabolism of acetate-glucose mixtures is simply an overlay ofglucose and acetate metabolism or whether metabolism of thesesubstrate mixtures is characterized by a unique metabolic pattern,we performed metabolic fluxanalyses.

Catabolism of glucose to PEP/pyruvate during growth on acetate-glucose mixtures differed considerably from that during growthon glucose alone. During growth on glucose, the glycolytic formationof PEP and pyruvate from glyceraldehyde-3-phosphate (227 mU ·[mg of protein]¹) was about 1.5-fold higher than the glucose uptake rate, whichis in good agreement with previous studies on glucose-grown strainsof C. glutamicum (26, 27, 28, 34, 49). Comparison ofgrowth on glucose to growth on acetate plus glucose shows thatthe glucose uptake was reduced twofold, but the glycolytic formationof PEP/pyruvate from glyceraldehyde-3-phosphate was reduced fourfold.This reflects the fact that on acetate-glucose mixtures, glucosepredominantly serves to generate precursors for biosyntheses startingwith glycolytic intermediates, and the proportion of carbon oxidizedto acetyl-CoA is greatly diminished compared to that during growthon glucose as a sole carbon source. Acetyl-CoA was derived almostexclusively from acetate when C. glutamicum was grown on acetateplus glucose (Fig. 4). The flux via the pentose phosphate shunthas been shown to be low when fructose is the sole carbon source(8) but high during growth on glucose (see also reference 26).Whereas it was low with acetate as the sole carbon source, fluxvia the pentose phosphate shunt is also high during growth onacetate-glucosemixtures.

The TCA cycle enzymes showed increasing in vivo activities in comparisons of growth on glucose, on glucose plus acetate, andon acetate (e.g., citrate synthase activity, 111, 219, and 413mU · [mg of protein]¹, respectively). In C. glutamicum, citrate synthase levels varylittle with the carbon source (specific activities in crude extracts,about 0.8 U · [mg of protein]¹) and the enzyme is inhibited by high concentrations of ATP andcis-aconitate (12). As its K_m value for acetyl-CoA of 51 µM(12) is higher than the intracellular concentration of acetyl-CoAduring growth on glucose but lower than that during growth onacetate (24 and 145 µM, respectively [53]), the in vivo activitiesof citrate synthase can be explained at least in part by the availabilityof the substrate acetyl-CoA.

C. glutamicum possesses two anaplerotic enzymes, PEP carboxylase and pyruvate carboxylase (31, 32, 33). During growthon glucose, PEP carboxylase and/or pyruvate carboxylase replenishesthe TCA cycle with precursors for biosyntheses requiring TCA cycleintermediates. Besides the net conversion of PEP and pyruvateto oxaloacetate and malate of 30 mU · (mg of protein)¹, an exchange rate of 102 mU · (mg of protein)¹ could be determined, corroborating the findings of Marx et al.(27), who showed that during growth of C. glutamicum strainLE4 on glucose, the PEP/pyruvate-oxaloacetate/malate interconversionamounts to about twice the net flux towards PEP/pyruvate (27).It remains to be shown whether these exchange reactions constitutea futile cycle or whether a reaction cycle of ATP-dependent pyruvatecarboxylase, NAD-dependent malate dehydrogenase, and NADPH-dependentmalic enzyme replaces transhydrogenase as has been proposed (8,18). The exchange reactions interconverting PEP/pyruvate andmalate/oxaolacetate were also present when C. glutamicum was grownon either acetate or glucose plus acetate (54 and 61 mU · [mgof protein]¹, respectively). However, during growth on acetate or glucoseplus acetate, there was no net formation of oxaloacetate/malatefrom PEP/pyruvate, but opposite, gluconeogenetic fluxes of 72and 15 mU · (mg of protein)¹ were determined (Fig. 3 and 4). The fact that pyruvate carboxylaseand PEP carboxylase did not serve an anaplerotic role during thegrowth of C. glutamicum on glucose plus acetate is surprisingand could not be predicted from the measurements of enzyme levels,as both pyruvate carboxylase and PEP carboxylase show similarenzyme levels during growth on acetate compared to growth on glucose.Our finding is consistent with the acetyl-CoA inhibition of pyruvatecarboxylase from C. glutamicum (K_i, 110 µM [32]) and an intracellularacetyl-CoA concentration of about 150 µM during growth on glucoseplus acetate (53). PEP carboxylase of C. glutamicum is inhibitedby aspartate (10), and it is possible that during growth onacetate or on glucose plus acetate, the intracellular aspartatepool is high due to sufficient formation of malate by the glyoxylatecycle and thus PEP carboxylase would also be inhibited. In orderto completely comprehend the complex PEP/pyruvate branch pointin corynebacterial metabolism, an experimental approach allowingthe quantitative determination of which enzymes, and to whichextent, are involved in the (inter)conversion of PEP/pyruvateand oxaloacetate/malate, will have to be pursued. Such an approachwill include genetic analyses as well as ¹³C isotopomer analyses (3, 47; A. A. de Graaf, V. F. Wendisch,and H. Sahm, Abstr. XVIIth Int. Conf. Magn. Reson. Biol. Syst.,abstr. TP25, 1996) that still need optimization before their applicationto complex metabolicsystems.

The glyoxylate cycle constitutes an anaplerotic sequence alternative to carboxylation of PEP and/or pyruvate (18). In C.glutamicum the glyoxylate cycle is inactive during growth on glucose,and the metabolization of isocitrate in the TCA cycle mainly servesenergy generation (Fig. 3). During growth on acetate, isocitrateis a metabolic branch point; 24% of isocitrate is fueled intothe glyoxylate cycle, and 76% is converted further in the TCAcycle (Fig. 2). Metabolic fluxes at this branch point have alsobeen determined in acetate-grown E. coli, and a similar relativeconversion of isocitrate was found (28% via the glyoxylate cycleand 72% via isocitrate dehydrogenase [24, 50]). However, forgrowth on glucose plus acetate, the metabolic fluxes at the isocitratebranch point in both organisms clearly differ. In E. coli, theglyoxylate cycle is inactive in vivo under this condition (51),but surprisingly, the glyoxylate cycle is active in C. glutamicum(isocitrate conversion by the glyoxylate cycle and isocitratedehydrogenase shows a relation of 23/77 [Fig. 4]). This differencebetween E. coli and C. glutamicum metabolism cannot be accountedfor by the substrate affinities of the respective enzymes, asthose are comparable (13, 35, 50), but is most probablydue to differing regulatory control. In E. coli, the genes codingfor isocitrate lyase (aceA) and malate synthase (aceB) are partof the aceBAK operon, which is repressed in the presence of glucosebut derepressed during growth on acetate or fatty acids (reviewedin reference 5). aceK codes for the bifunctional isocitratedehydrogenase kinase/phosphatase, which controls the phosphorylationstatus of isocitrate dehydrogenase (14, 22). Thus, duringgrowth on acetate, there are high levels of isocitrate lyase andmalate synthase, while isocitrate dehydrogenase is predominantlyin its inactive, phosphorylated form. During the growth of E.coli on glucose-acetate mixtures, lower isocitrate lyase and malatesynthase levels are present and isocitrate dehydrogenase is mostlyin its active, unphosphorylated form. In C. glutamicum, however,there is no evidence for a similar modificatory control of isocitratedehydrogenase, and transcription of the isocitrate lyase and malatesynthase genes, which are not part of an operon, is increasedin the presence of acetate regardless of the presence or absenceof glucose (53). The relative metabolization of isocitrate byisocitrate dehydrogenase and by isocitrate lyase (76 to 24%) isconsistent with their K_m values of 12 and 280 µM, respectively,and allosteric regulation by glyoxylate and oxaloacetate (13,35).

The quantitative determination of metabolic fluxes presented here led to the hypothesis that a glyoxylate cycle-deficientstrain of C. glutamicum should be impaired in growth on glucose-acetatemixtures. To test this hypothesis, strain WT $Delta$ AB, which is devoidof isocitrate lyase and malate synthase activities, was constructedby targeted deletion of the aceA-aceB gene cluster on the C. glutamicumchromosome. In this strain accumulation of glyoxylate and sidereactions of malate synthase such as might occur in the malatesynthase-deficient strain ALB1 and the isocitrate lyase-deficientstrain ASK1, respectively (35, 36), are avoided. Indeed, theglyoxylate cycle-deficient strain WT $Delta$ AB could cometabolize glucoseand acetate but showed longer doubling times during growth onglucose-acetate mixtures than the WT. Thus, during growth on glucoseplus acetate, PEP carboxylase and pyruvate carboxylase can onlypartly fulfill the anaplerotic function in C. glutamicum. Clearly,the glyoxylate cycle is required for optimal growth of C. glutamicumon glucose-acetate mixtures, verifying the physiological effectof this pathway alteration as predicted from our metabolic fluxanalyses.

	ACKNOWLEDGMENTS

We thank Petra Peters-Wendisch and Lothar Eggeling for critical reading of the manuscript and Achim Marx fordiscussions.

This work was supported by EU grant BIO 4-CT96-0145. V.F.W. was a fellow of the Deutsche Forschungsgemeinschaft (DFG)-Graduiertenkolleg'Molekulare Physiologie: Stoff- und Energieumwandlung' at theHeinrich-Heine-Universität Düsseldorf, Düsseldorf,Germany.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Biotechnology 1, Research Center Jülich, D-52428 Jülich, Germany, Phone:49-2461-615169. Fax: 49-2461-612710. E-mail: v.wendisch{at}fz-juelich.de.

Dedicated to Rudolf K. Thauer on the occasion of his 60thbirthday.

Present address: Abt. Mikrobiologie und Biotechnologie, University of Ulm, D-89061 Ulm,Germany.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Axe, D. D., and J. E. Bailey. 1995. Transport of lactate and acetate through the energized cytoplasmic membrane of Escherichia coli. Biotechnol. Bioeng. 47:8-19[CrossRef].

2. Baronofsky, J. J., W. J. A. Schreurs, and E. R. Kashket. 1984. Uncoupling by acetic acid limits growth of and acetogenesis by Clostridium thermoaceticum. Appl. Environ. Microbiol. 48:1134-1139[Abstract/Free Full Text].

3. Beale, J. M., and J. L. Foster. 1996. Carbohydrate fluxes into alginate biosynthesis in Azotobacter vinelandii NCIB 8789: NMR investigations of the triose pools. Biochemistry 35:4492-4501[CrossRef][Medline].

4. Brown, T. D. K., M. C. Jones-Mortimer, and H. L. Kornberg. 1977. The enzymatic interconversion of acetate and acetyl-coenzyme A in Escherichia coli. J. Gen. Microbiol. 102:327-336[Medline].

5. Clark, D. P., and J. E. Cronan. 1996. Two-carbon compounds and fatty acids as carbon sources, p. 343-357. In F. C. Neidhardt, R. Curtiss III, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed. American Society for Microbiology, Washington, D.C.

6. Cocaign, M., C. Monnet, and N. D. Lindley. 1993. Batch kinetics of Corynebacterium glutamicum during growth on various substrates: use of substrate mixtures to localize metabolic bottlenecks. Appl. Microbiol. Biotechnol. 40:526-530[CrossRef].

7. Dominguez, H., M. Cocaign-Bousquet, and N. D. Lindley. 1993. Simultaneous consumption of glucose and fructose from sugar mixtures during batch growth of Corynebacterium glutamicum. Appl. Microbiol. Biotechnol. 47:600-603[CrossRef].

8. Dominguez, H., C. Rollin, A. Guyonvarch, J. L. Guerquin-Kern, M. Cocaign-Bousquet, and N. D. Lindley. 1998. Carbon flux distribution in the central metabolic pathways of Corynebacterium glutamicum during growth on fructose. Eur. J. Biochem. 254:96-102[Medline].

9. Ebbighausen, H., B. Weil, and R. Krämer. 1991. Carrier-mediated acetate uptake in Corynebacterium glutamicum. Arch. Microbiol. 155:505-510[CrossRef].

10. Eikmanns, B. J., M. T. Follettie, M. U. Griot, and A. J. Sinskey. 1989. The phosphoenolpyruvate carboxylase gene of Corynebacterium glutamicum: molecular cloning, nucleotide sequence, and expression. Mol. Gen. Genet. 218:330-339[CrossRef][Medline].

11. Eikmanns, B. J., M. Metzger, D. J. Reinscheid, and H. Sahm. 1991. Amplification of three threonine biosynthesis genes in Corynebacterium glutamicum and its influence on carbon flux in different strains. Appl. Microbiol. Biotechnol. 102:93-98.

12. Eikmanns, B. J., N. Thum-Schmitz, L. Eggeling, K. Lüdtke, and H. Sahm. 1994. Nucleotide sequence, expression, and transcriptional analysis of the Corynebacterium glutamicum gltA gene encoding citrate synthase. Microbiology 140:1817-1828[Abstract].

13. Eikmanns, B. J., D. Rittmann, and H. Sahm. 1995. Cloning, sequence analysis, expression, and inactivation of the Corynebacterium glutamicum icd gene encoding isocitrate dehydrogenase and biochemical characterization of the enzyme. J. Bacteriol. 177:774-782[Abstract/Free Full Text].

14. Garnak, M., and H. C. Reeves. 1979. Phosphorylation of isocitrate dehydrogenase of Escherichia coli. Science 203:1111-1112[Abstract/Free Full Text].

15. George, S. E., C. J. Costenbader, and T. Melton. 1985. Diauxic growth in Azotobacter vinelandii. J. Bacteriol. 164:866-871[Abstract/Free Full Text].

16. Harder, W., and L. Dijkhuizen. 1982. Strategies of mixed substrate utilization in microorganisms. Phil. Trans. R. Soc. Lond. 297:459-480[Medline].

17. Kinoshita, S., and K. Tanaka. 1972. Glutamic acid, p. 263-324. In K. Yamada (ed.), The microbial production of amino acids. John Wiley, New York, N.Y.

18. Kornberg, H. L. 1966. The role and control of the glyoxylate cycle in Escherichia coli. Biochem. J. 99:1-11[Medline].

19. Koshland, D. E., Jr. 1998. The era of pathway quantification. Science 280:852-853[Free Full Text].

20. Kovarova-Kovar, K., and T. Egli. 1998. Growth kinetics of suspended microbial cells: from single-substrate-controlled growth to mixed-substrate kinetics. Microbiol. Mol. Biol. Rev. 62:646-666[Abstract/Free Full Text].

21. Krämer, R., C. Lambert, C. Hoischen, and H. Ebbighausen. 1990. Uptake of glutamate in Corynebacterium glutamicum. 1. Kinetic properties and regulation by internal pH and potassium. Eur. J. Biochem. 194:929-935[Medline].

22. LaPorte, D. C., and D. E. Koshland, Jr. 1982. A protein with kinase and phosphatase activities involved in regulation of the tricarboxylic acid cycle. Nature 300:458-460[CrossRef][Medline].

23. Liebl, W. 1991. The genus Corynebacterium $---$ nonmedical, p. 1157-1171. In A. Balows, H. G. Trüper, M. Dworkin, W. Harder, and K. H. Schleifer (ed.), The procaryotes, vol. 2. Springer, New York, N.Y.

24. London, R. E. 1988. ¹³C labeling in studies of metabolic regulation. Prog. NMR Spectrosc. 20:337-383.

25. Lundberg, P., E. Harmsen, C. Ho, and H. J. Vogel. 1990. Nuclear magnetic resonance studies of cellular metabolism. Anal. Biochem. 191:193-222[CrossRef][Medline].

26. Marx, A., A. A. de Graaf, W. Wiechert, L. Eggeling, and H. Sahm. 1996. Determination of the fluxes in the central metabolism of Corynebacterium glutamicum by nuclear magnetic resonance spectroscopy combined with metabolite balancing. Biotechnol. Bioeng. 49:111-129[CrossRef].

27. Marx, A., K. Striegel, A. A. de Graaf, H. Sahm, and L. Eggeling. 1997. Response of the central metabolism of Corynebacterium glutamicum to different flux burdens. Biotechnol. Bioeng. 56:168-180[CrossRef].

28. Marx, A., B. J. Eikmanns, H. Sahm, and A. A. de Graaf. 1999. Response of the central metabolism in Corynebacterium glutamicum to the use of an NADH-dependent glutamate dehydrogenase. Metab. Eng. 1:35-48[CrossRef][Medline].

29. Monod, J. 1949. The growth of bacterial cultures. Annu. Rev. Microbiol. 3:371-394[CrossRef].

30. Peters-Wendisch, P. G., B. J. Eikmanns, G. Thierbach, B. Bachmann, and H. Sahm. 1993. Phosphoenolpyruvate carboxylase in Corynebacterium glutamicum is dispensable for growth and lysine production. FEMS Microbiol. Lett. 112:269-274[CrossRef].

31. Peters-Wendisch, P. G., V. F. Wendisch, A. A. de Graaf, B. J. Eikmanns, and H. Sahm. 1996. C₃-carboxylation as an anaplerotic reaction in phosphoenolpyruvate carboxylase-deficient Corynebacterium glutamicum. Arch. Microbiol. 165:387-396[CrossRef][Medline].

32. Peters-Wendisch, P. G., V. F. Wendisch, S. Paul, B. J. Eikmanns, and H. Sahm. 1997. Pyruvate carboxylase as an anaplerotic enzyme in Corynebacterium glutamicum. Microbiology 143:1095-1103.

33. Peters-Wendisch, P. G., C. Kreutzer, J. Kalinowski, M. Patek, H. Sahm, and B. J. Eikmanns. 1998. Pyruvate carboxylase from Corynebacterium glutamicum: characterization, expression and inactivation of the pyc gene. Microbiology 144:915-927[Abstract].

34. Pons, A., C. G. Dussap, C. Pequinot, and J. B. Gros. 1996. Metabolic flux distribution in Corynebacterium melassecola ATCC 17965 for various carbon sources. Biotechnol. Bioeng. 51:177-189.

35. Reinscheid, D. J., B. J. Eikmanns, and H. Sahm. 1994. Characterization of the isocitrate lyase gene from Corynebacterium glutamicum and biochemical analysis of the enzyme. J. Bacteriol. 176:3474-3483[Abstract/Free Full Text].

36. Reinscheid, D. J., B. J. Eikmanns, and H. Sahm. 1994. Malate synthase from Corynebacterium glutamicum: sequence analysis of the gene and biochemical characterization of the enzyme. Microbiology 140:3099-3108[Abstract].

37. Reinscheid, D. J., S. Schnicke, D. Rittmann, U. Zahnow, H. Sahm, and B. J. Eikmanns. 1999. Cloning, sequence analysis, expression and inactivation of the Corynebacterium glutamicum pta-ack operon encoding phosphotransacetylase and acetate kinase. Microbiology 145:503-513[Abstract].

38. Salou, P., P. Loubiere, and A. Pareilleux. 1994. Growth and energetics of Leuconostoc oenos during cometabolism of glucose with citrate or fructose. Appl. Environ. Microbiol. 60:1459-1466[Abstract/Free Full Text].

39. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

40. Schäfer, A., A. Tauch, W. Jäger, J. Kalinowski, G. Thierbach, and A. Pühler. 1994. Small mobilizable multi-purpose cloning vectors derived from the Escherichia coli plasmids pK18 and pK19: selection of defined deletions in the chromosome of Corynebacterium glutamicum. Gene 145:69-73[CrossRef][Medline].

41. Scharfstein, S. T., S. N. Tucker, A. Mancuso, H. W. Blanch, and D. S. Clark. 1994. Quantitative in vivo nuclear magnetic resonance studies of hybridoma metabolism. Biotechnol. Bioeng. 43:1059-1074[CrossRef].

42. Schrumpf, B., A. Schwarzer, J. Kalinowski, A. Pühler, L. Eggeling, and H. Sahm. 1991. A functional split pathway for lysine synthesis in Corynebacterium glutamicum. J. Bacteriol. 173:4510-4516[Abstract/Free Full Text].

43. Sequin, U., and A. I. Scott. 1974. Carbon-13 as a label in biosynthetic studies. Science 186:101-107[Free Full Text].

44. Sonntag, K., L. Eggeling, A. A. de Graaf, and H. Sahm. 1995. Flux partitioning in the split pathway of lysine synthesis in Corynebacterium. Eur. J. Biochem. 213:1325-1331[Medline].

45. Sonntag, K., J. Schwinde, A. A. de Graaf, A. Marx, B. J. Eikmanns, W. Wiechert, and H. Sahm. 1995. ¹³C NMR studies of the fluxes in the central metabolism of Corynebacterium glutamicum during growth and overproduction of amino acids in batch cultures. Appl. Microbiol. Biotechnol. 44:489-495[CrossRef].

46. Stephanopoulos, G., and J. J. Vallino. 1991. Network rigidity and metabolic engineering in metabolite overproduction. Science 252:1675-1681[Abstract/Free Full Text].

47. Szyperski, T. 1996. Biosynthetically directed fractional ¹³C-labeling of proteinogenic amino acids. Eur. J. Biochem. 232:433-448[Medline].

48. Tauchert, K., A. Jahn, and J. Oelze. 1990. Control of diauxic growth of Azotobacter vinelandii on acetate and glucose. J. Bacteriol. 172:6447-6451[Abstract/Free Full Text].

49. Vallino, J. J., and G. Stephanopoulos. 1993. Metabolic flux distributions in Corynebacterium glutamicum during growth and lysine overproduction. Biotechnol. Bioeng. 41:633-646[CrossRef].

50. Walsh, K., and D. E. Koshland, Jr. 1984. Determination of flux through the branch point of two metabolic cycles. J. Biol. Chem. 259:9646-9654[Abstract/Free Full Text].

51. Walsh, K., and D. E. Koshland, Jr. 1985. Branch point control by the phosphorylation state of isocitrate dehydrogenase. J. Biol. Chem. 260:8430-8437[Abstract/Free Full Text].

52. Wendisch, V. F., A. A. de Graaf, and H. Sahm. 1997. Accurate determination of ¹³C enrichments in nonprotonated carbon atoms of isotopically enriched amino acids by ¹H nuclear magnetic resonance. Anal. Biochem. 245:196-202[CrossRef][Medline].

53. Wendisch, V. F., M. Spies, D. J. Reinscheid, S. Schnicke, H. Sahm, and B. J. Eikmanns. 1997. Regulation of acetate metabolism in Corynebacterium glutamicum: transcriptional control of the isocitrate lyase and malate synthase genes. Arch. Microbiol. 168:262-269[CrossRef][Medline].

54. Wiechert, W., and A. A. de Graaf. 1997. Bidirectional reaction steps in metabolic networks. Part I. Modeling and simulation of carbon labelling experiments. Biotechnol. Bioeng. 55:101-117[CrossRef].

55. Wiechert, W., C. Siefke, A. Marx, and A. A. de Graaf. 1997. Bidirectional reaction steps in metabolic networks. Part II. Flux estimation and statistical analysis. Biotechnol. Bioeng. 55:118-135[CrossRef].

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4.	Brown, T. D. K., M. C. Jones-Mortimer, and H. L. Kornberg. 1977. The enzymatic interconversion of acetate and acetyl-coenzyme A in Escherichia coli. J. Gen. Microbiol. 102:327-336[Medline].
5.	Clark, D. P., and J. E. Cronan. 1996. Two-carbon compounds and fatty acids as carbon sources, p. 343-357. In F. C. Neidhardt, R. Curtiss III, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. S. Reznikoff, M. Riley, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed. American Society for Microbiology, Washington, D.C.
6.	Cocaign, M., C. Monnet, and N. D. Lindley. 1993. Batch kinetics of Corynebacterium glutamicum during growth on various substrates: use of substrate mixtures to localize metabolic bottlenecks. Appl. Microbiol. Biotechnol. 40:526-530[CrossRef].
7.	Dominguez, H., M. Cocaign-Bousquet, and N. D. Lindley. 1993. Simultaneous consumption of glucose and fructose from sugar mixtures during batch growth of Corynebacterium glutamicum. Appl. Microbiol. Biotechnol. 47:600-603[CrossRef].
8.	Dominguez, H., C. Rollin, A. Guyonvarch, J. L. Guerquin-Kern, M. Cocaign-Bousquet, and N. D. Lindley. 1998. Carbon flux distribution in the central metabolic pathways of Corynebacterium glutamicum during growth on fructose. Eur. J. Biochem. 254:96-102[Medline].
9.	Ebbighausen, H., B. Weil, and R. Krämer. 1991. Carrier-mediated acetate uptake in Corynebacterium glutamicum. Arch. Microbiol. 155:505-510[CrossRef].
10.	Eikmanns, B. J., M. T. Follettie, M. U. Griot, and A. J. Sinskey. 1989. The phosphoenolpyruvate carboxylase gene of Corynebacterium glutamicum: molecular cloning, nucleotide sequence, and expression. Mol. Gen. Genet. 218:330-339[CrossRef][Medline].
11.	Eikmanns, B. J., M. Metzger, D. J. Reinscheid, and H. Sahm. 1991. Amplification of three threonine biosynthesis genes in Corynebacterium glutamicum and its influence on carbon flux in different strains. Appl. Microbiol. Biotechnol. 102:93-98.
12.	Eikmanns, B. J., N. Thum-Schmitz, L. Eggeling, K. Lüdtke, and H. Sahm. 1994. Nucleotide sequence, expression, and transcriptional analysis of the Corynebacterium glutamicum gltA gene encoding citrate synthase. Microbiology 140:1817-1828[Abstract].
13.	Eikmanns, B. J., D. Rittmann, and H. Sahm. 1995. Cloning, sequence analysis, expression, and inactivation of the Corynebacterium glutamicum icd gene encoding isocitrate dehydrogenase and biochemical characterization of the enzyme. J. Bacteriol. 177:774-782[Abstract/Free Full Text].
14.	Garnak, M., and H. C. Reeves. 1979. Phosphorylation of isocitrate dehydrogenase of Escherichia coli. Science 203:1111-1112[Abstract/Free Full Text].
15.	George, S. E., C. J. Costenbader, and T. Melton. 1985. Diauxic growth in Azotobacter vinelandii. J. Bacteriol. 164:866-871[Abstract/Free Full Text].
16.	Harder, W., and L. Dijkhuizen. 1982. Strategies of mixed substrate utilization in microorganisms. Phil. Trans. R. Soc. Lond. 297:459-480[Medline].
17.	Kinoshita, S., and K. Tanaka. 1972. Glutamic acid, p. 263-324. In K. Yamada (ed.), The microbial production of amino acids. John Wiley, New York, N.Y.
18.	Kornberg, H. L. 1966. The role and control of the glyoxylate cycle in Escherichia coli. Biochem. J. 99:1-11[Medline].
19.	Koshland, D. E., Jr. 1998. The era of pathway quantification. Science 280:852-853[Free Full Text].
20.	Kovarova-Kovar, K., and T. Egli. 1998. Growth kinetics of suspended microbial cells: from single-substrate-controlled growth to mixed-substrate kinetics. Microbiol. Mol. Biol. Rev. 62:646-666[Abstract/Free Full Text].
21.	Krämer, R., C. Lambert, C. Hoischen, and H. Ebbighausen. 1990. Uptake of glutamate in Corynebacterium glutamicum. 1. Kinetic properties and regulation by internal pH and potassium. Eur. J. Biochem. 194:929-935[Medline].
22.	LaPorte, D. C., and D. E. Koshland, Jr. 1982. A protein with kinase and phosphatase activities involved in regulation of the tricarboxylic acid cycle. Nature 300:458-460[CrossRef][Medline].
23.	Liebl, W. 1991. The genus Corynebacterium $---$ nonmedical, p. 1157-1171. In A. Balows, H. G. Trüper, M. Dworkin, W. Harder, and K. H. Schleifer (ed.), The procaryotes, vol. 2. Springer, New York, N.Y.
24.	London, R. E. 1988. ¹³C labeling in studies of metabolic regulation. Prog. NMR Spectrosc. 20:337-383.
25.	Lundberg, P., E. Harmsen, C. Ho, and H. J. Vogel. 1990. Nuclear magnetic resonance studies of cellular metabolism. Anal. Biochem. 191:193-222[CrossRef][Medline].
26.	Marx, A., A. A. de Graaf, W. Wiechert, L. Eggeling, and H. Sahm. 1996. Determination of the fluxes in the central metabolism of Corynebacterium glutamicum by nuclear magnetic resonance spectroscopy combined with metabolite balancing. Biotechnol. Bioeng. 49:111-129[CrossRef].
27.	Marx, A., K. Striegel, A. A. de Graaf, H. Sahm, and L. Eggeling. 1997. Response of the central metabolism of Corynebacterium glutamicum to different flux burdens. Biotechnol. Bioeng. 56:168-180[CrossRef].
28.	Marx, A., B. J. Eikmanns, H. Sahm, and A. A. de Graaf. 1999. Response of the central metabolism in Corynebacterium glutamicum to the use of an NADH-dependent glutamate dehydrogenase. Metab. Eng. 1:35-48[CrossRef][Medline].
29.	Monod, J. 1949. The growth of bacterial cultures. Annu. Rev. Microbiol. 3:371-394[CrossRef].
30.	Peters-Wendisch, P. G., B. J. Eikmanns, G. Thierbach, B. Bachmann, and H. Sahm. 1993. Phosphoenolpyruvate carboxylase in Corynebacterium glutamicum is dispensable for growth and lysine production. FEMS Microbiol. Lett. 112:269-274[CrossRef].
31.	Peters-Wendisch, P. G., V. F. Wendisch, A. A. de Graaf, B. J. Eikmanns, and H. Sahm. 1996. C₃-carboxylation as an anaplerotic reaction in phosphoenolpyruvate carboxylase-deficient Corynebacterium glutamicum. Arch. Microbiol. 165:387-396[CrossRef][Medline].
32.	Peters-Wendisch, P. G., V. F. Wendisch, S. Paul, B. J. Eikmanns, and H. Sahm. 1997. Pyruvate carboxylase as an anaplerotic enzyme in Corynebacterium glutamicum. Microbiology 143:1095-1103.
33.	Peters-Wendisch, P. G., C. Kreutzer, J. Kalinowski, M. Patek, H. Sahm, and B. J. Eikmanns. 1998. Pyruvate carboxylase from Corynebacterium glutamicum: characterization, expression and inactivation of the pyc gene. Microbiology 144:915-927[Abstract].
34.	Pons, A., C. G. Dussap, C. Pequinot, and J. B. Gros. 1996. Metabolic flux distribution in Corynebacterium melassecola ATCC 17965 for various carbon sources. Biotechnol. Bioeng. 51:177-189.
35.	Reinscheid, D. J., B. J. Eikmanns, and H. Sahm. 1994. Characterization of the isocitrate lyase gene from Corynebacterium glutamicum and biochemical analysis of the enzyme. J. Bacteriol. 176:3474-3483[Abstract/Free Full Text].
36.	Reinscheid, D. J., B. J. Eikmanns, and H. Sahm. 1994. Malate synthase from Corynebacterium glutamicum: sequence analysis of the gene and biochemical characterization of the enzyme. Microbiology 140:3099-3108[Abstract].
37.	Reinscheid, D. J., S. Schnicke, D. Rittmann, U. Zahnow, H. Sahm, and B. J. Eikmanns. 1999. Cloning, sequence analysis, expression and inactivation of the Corynebacterium glutamicum pta-ack operon encoding phosphotransacetylase and acetate kinase. Microbiology 145:503-513[Abstract].
38.	Salou, P., P. Loubiere, and A. Pareilleux. 1994. Growth and energetics of Leuconostoc oenos during cometabolism of glucose with citrate or fructose. Appl. Environ. Microbiol. 60:1459-1466[Abstract/Free Full Text].
39.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
40.	Schäfer, A., A. Tauch, W. Jäger, J. Kalinowski, G. Thierbach, and A. Pühler. 1994. Small mobilizable multi-purpose cloning vectors derived from the Escherichia coli plasmids pK18 and pK19: selection of defined deletions in the chromosome of Corynebacterium glutamicum. Gene 145:69-73[CrossRef][Medline].
41.	Scharfstein, S. T., S. N. Tucker, A. Mancuso, H. W. Blanch, and D. S. Clark. 1994. Quantitative in vivo nuclear magnetic resonance studies of hybridoma metabolism. Biotechnol. Bioeng. 43:1059-1074[CrossRef].
42.	Schrumpf, B., A. Schwarzer, J. Kalinowski, A. Pühler, L. Eggeling, and H. Sahm. 1991. A functional split pathway for lysine synthesis in Corynebacterium glutamicum. J. Bacteriol. 173:4510-4516[Abstract/Free Full Text].
43.	Sequin, U., and A. I. Scott. 1974. Carbon-13 as a label in biosynthetic studies. Science 186:101-107[Free Full Text].
44.	Sonntag, K., L. Eggeling, A. A. de Graaf, and H. Sahm. 1995. Flux partitioning in the split pathway of lysine synthesis in Corynebacterium. Eur. J. Biochem. 213:1325-1331[Medline].
45.	Sonntag, K., J. Schwinde, A. A. de Graaf, A. Marx, B. J. Eikmanns, W. Wiechert, and H. Sahm. 1995. ¹³C NMR studies of the fluxes in the central metabolism of Corynebacterium glutamicum during growth and overproduction of amino acids in batch cultures. Appl. Microbiol. Biotechnol. 44:489-495[CrossRef].
46.	Stephanopoulos, G., and J. J. Vallino. 1991. Network rigidity and metabolic engineering in metabolite overproduction. Science 252:1675-1681[Abstract/Free Full Text].
47.	Szyperski, T. 1996. Biosynthetically directed fractional ¹³C-labeling of proteinogenic amino acids. Eur. J. Biochem. 232:433-448[Medline].
48.	Tauchert, K., A. Jahn, and J. Oelze. 1990. Control of diauxic growth of Azotobacter vinelandii on acetate and glucose. J. Bacteriol. 172:6447-6451[Abstract/Free Full Text].
49.	Vallino, J. J., and G. Stephanopoulos. 1993. Metabolic flux distributions in Corynebacterium glutamicum during growth and lysine overproduction. Biotechnol. Bioeng. 41:633-646[CrossRef].
50.	Walsh, K., and D. E. Koshland, Jr. 1984. Determination of flux through the branch point of two metabolic cycles. J. Biol. Chem. 259:9646-9654[Abstract/Free Full Text].
51.	Walsh, K., and D. E. Koshland, Jr. 1985. Branch point control by the phosphorylation state of isocitrate dehydrogenase. J. Biol. Chem. 260:8430-8437[Abstract/Free Full Text].
52.	Wendisch, V. F., A. A. de Graaf, and H. Sahm. 1997. Accurate determination of ¹³C enrichments in nonprotonated carbon atoms of isotopically enriched amino acids by ¹H nuclear magnetic resonance. Anal. Biochem. 245:196-202[CrossRef][Medline].
53.	Wendisch, V. F., M. Spies, D. J. Reinscheid, S. Schnicke, H. Sahm, and B. J. Eikmanns. 1997. Regulation of acetate metabolism in Corynebacterium glutamicum: transcriptional control of the isocitrate lyase and malate synthase genes. Arch. Microbiol. 168:262-269[CrossRef][Medline].
54.	Wiechert, W., and A. A. de Graaf. 1997. Bidirectional reaction steps in metabolic networks. Part I. Modeling and simulation of carbon labelling experiments. Biotechnol. Bioeng. 55:101-117[CrossRef].
55.	Wiechert, W., C. Siefke, A. Marx, and A. A. de Graaf. 1997. Bidirectional reaction steps in metabolic networks. Part II. Flux estimation and statistical analysis. Biotechnol. Bioeng. 55:118-135[CrossRef].